ProductDescription
SphereCol®beadsarecoatedwithVitroCol®humanTypeIcollagenandareidealforgrowingcellsinsUSPension.Thecollagencoatedbeadsprovideanaturalinvivo-likeenvironmenttopromotehighcellgrowthwhileprovidingalargesurfaceareaforcellstoattachwithoptimalsurfaceareatovolumeratios.SphereCol®providesa3Dbio-scaffoldwhichisoptimalinmanycellcultureprocedures.
SphereCol®,humancollagencoatedbeadsiscoatedwithhighlypurifiedTypeIhumancollagenderivedfromahumanfibroblastcellcultureprocess,VitroCol®.Thecollagenprovidesanoptimalcoatingonthebeadstoenhancecellattachment,cellviABIlity,cellproliferationandcellfunction.Thecollagenbeadsrangeinsizefromabout125to250micron.Theproductispackagedina20mlbottleandsterilized.SphereCol®isprovidedinauser-friendlypackagingforuseandstorage.
| Parameter,Testing,andMethod | SphereCol®#5138 |
| BeadShape | Spherical |
| PackageSize | 10grams |
| BeadsperGram | 4.6x105 |
| BeadSizeDistribution | 125-250microns |
RelativeDensityRange | 1.022-1.030 |
| SurfaceAreaperBead | 360cm2/gram |
| CollagenUsedforCoating | VitroCol®HumanTypeICollagen |
| StorageTemperature | RoomTemperature |
| ShelfLife | Minimumof6monthsfromdateofreceipt |
| SterilizationMethod | IrrADIation |
DirectionsforUse
DownloadthefullPDFversionorcontinuereadingbelow:
Note:SphereColisprovidedasasterile,drypowderandthusmustbehandledinanasepticmanner.
Theinstructionsbelowaredesignedtoserveasageneralguidelineforthecultureofa200mlspinnercontainingaSphereCol®,humancollagenbeadsataconcentrationof5cm2/mlataseedingdensityof20,000cells/cm2utilizingalowserumattachmentphase(i.e.,0.05%FBS-containingmedium).
Preparation
- Weighout2.78grams(1000cm2)oftheSphereCol®beadsandaddthemtoasterilized250mlspinnerflask.Note:WeighouttheappropriatemassofSphereCol®beadsintoasteriletube.AddavolumeofsterilePBSormediumsuchthatthemassofbeads(andthus,surfacearea)pervolumeisknown.Aliquotthedesiredmassintoasterilevessel.Youmayremovetheliquidbycarefullydecantingoraspirating.
- Add180mloflowserum-containingcellculturemedium(i.e.,0.05%)tothespinnerflask.Thisallowsfora10mladditionofcellinoculumfollowedbya10mladditionofFBSuponsatisfactorycellattachment.
Acclimation
- Tomaximizecellattachment,themediumandSphereCol®beadsmixtureshouldbeacclimatedtothecultureenvironmentpriortoaddingthecellinoculum.Forexample,placementofthevessel(i.e.,a200mlspinneronastirplate)ina37°C,5%CO2incubatorforaminimumof30minutesallowsfortemperature,gasandpHequilibration.
GenerateCellInoculum
- Harvestcellsusingstandardcellculturetechniquesandreagents.Note:Theexactprocedurerequiredtoproducetheoptimalcellinoculumwillvarybasedonthecelltypeandcellculturesystem.Ideally,auniform,single-cellsuspensionisdesiredtoallowforanevendistributionofcellsacrosstheSphereCol®beadspopulation.
- Uponachievingasatisfactorycellsuspension,transfer20X106cellstoacentrifugetube,spindownandre-suspendin10mllow-serumcellculturemedium.Note:20X106cellsacross1000cm2equatesto20,000cells/cm2
CellAttachmenttoSphereCol®Beads(“AttachmentPhase”)
- Removespinnerflaskfromincubatorandplaceonstirplateunderlaminarflowcabinet.
- Add10mlcellsuspensiontospinnerflask.
- Uponsatisfactorycellattachment,add10mlserumtobringthefinalconcentrationofserumto5%.Note:CellswilltypicallybegintoattachtoSphereCol®beadsoverthefirstfewhoursoftheculture,althoughthiswillvarybasedoncelltypeandcultureconditions.Ideally,theattachmentphaseisconsideredcompleteonce>90%ofcellsareattached,whichcanbeconfirmedmicroscopically(seeMonitoringandMaintainingtheCulture).
AdditionalConsiderations:
- Alow-serumattachmentphaseissometimesrequiredforcellsthatwilleithernotattachatall,ordonotattachinanevenlydistributedmannerinthepresenceofthestandardserumconcentrations.Theoptimalconcentrationofserumduringtheinitialattachmentphase(typicallythefirst1to4hours)mustbedeterminedforeachcellculturesystem.Oftentimesithasbeenfoundtobeverylow(i.e.,0.05%).Uponsatisfactorycellattachment,serummaybeaddedtothedesiredfinalconcentration.
- Anallowancefortheadditionofserumaftercellattachmentmustalsobeaccountedforifperformingalow-serumattachmentstep.
- AnevendistributionofcellsacrosstheSphereCol®beadspopulationiscriticalinmaximizingtheusageofavailablesurfacearea,leadingtomaximalcellyield.
- Agitationspeedisaprocessparameterthatrequiresoptimizationforgoodcellattachmentinspinners.Ataminimum,theagitationrateshouldbesufficienttoevenlysuspendtheSphereCol®beads.Ingeneral,thelowestagitationratethatallowsforgoodcellattachmentandevensuspensionofSphereCol®beadsshouldbechosen,soastolessensheerforcesexerteduponthecellsbythedynamicenvironmentofthespinner.
MonitoringandMaintainingtheCulture
- Theculturemaybemonitoredbycollectingrepresentativesamplesinculturedishes(i.e.,multiwellplates)andvisualizingunderamicroscope.Cellattachmentandspreadingcanbeeasilyobservedat100Xmagnificationatvarioustimepointsatwhichtimeaqualitativeassessmentoftheattachmentandspreadingcanbemade.CellscanbevisualizedattheedgesorcircumferenceoftheSphereCol®beadsasrounded(initialattachmentphase),“gumdrop-shaped”(earlyspreading)orflattened(completelyspread).
- Aswithflatcultureware,mediaexchangesmaybenecessarytomaintainastablesupplyofnutrientsoverthecourseoftheculture.Inalaminarflowhood,allowtheSphereCol®beadstosettletothebottomofthevesselandwithdrawthedesiredvolumeofmediumfromthetop,takingcarenottoremoveanySphereCol®beads.Replacewithanequalvolumeoffresh,warmedculturemedium.
AdditionalConsiderations:
- SeveraltechniquesmaybeusedtoenhancevisualizationofcellsonSphereCol®beadsifneeded:
- Fluorescencetechniques(i.e.,DAPIstainingmethod)
- Acridineorange
- Directvisualizationbyphasemicroscopy
- Asthecellsgrow,SphereCol®beadswillbecomeheavier,andtheagitationrate(inthecaseofaspinnerculture)mayneedtobeincreasedtomaintainauniformsuspension.
HarvestingCells
- WhilestandardcellharvestingreagentsandtechniquesusedforflatculturewaretypicallyworkwellwithSphereCol®beadscultures,harvestconditionswillneedtobeoptimizedforeachcelltypeandcellculturesystemtogetthebestresultspossIBLe.Optimalharvestconditionsinflatculturewareprovideagoodstartingpoint.Ingeneral,theconditionsgentlestonthecellsshouldbeused.
- Removethemediafromthespinner,beingcarefulnottoremovecell-ladenSphereCol®beads.
- WashtheSphereCol®beadswith40mlphosphatebufferedsaline(PBS).Incubateatroomtemperaturefor10minutes.
- AspiratePBS,andadd10mldissociationenzyme(i.e.,trypsin).AllowcellstoincubateintheenzymeuntiltheydissociatefromtheSphereCol®beadssurface,thentrituratetoobtainasinglecellsuspension.SphereCol®beads/cellsmaybeplacedat37°Ctofacilitatedetachment.
- Countcellswithahemocytometerusingtrypanblue.SphereCol®beadsgenerallydonotgetunderthecoverslip,sotheywillnotinterferewiththecount.Keeptrackofallthereagentvolumesusedaswellasthemediavolumeremovedsothatthecellcountcanbeadjustedwiththeappropriatedilution/concentrationfactor.
AdditionalConsiderations:
- Washingisperformedtoaidintheremovaloftrypsininhibitingmediacomponents.SolutionsotherthanPBSarealsowellsuitedforthispurpose.
- Trypsinconditionsshouldbeasgentleaspossible,solongasasingle-cellsuspensionisobtainedinastimelyfashion.Highertrypsinconcentrations,longerincubationtimes,andhighertemperaturesaresomefactorsthatcouldnegativelyimpactcellhealth.
- Somecells,suchasMDCKcells,aredifficulttodissociate,andthereforerequireharshertechniques,suchastheuseof0.25%(5X)Trypsin-EDTA,andincubationat37°Cforover10minutes.ItmayalsobebeneficialtoperformanEDTAwashpriortotrypsinaddition.
- Foranimalcomponentderivedfreesystems,trypsinsubstitutes,suchasTrypLE,canbeusedtochemicallydissociatecells.
- ToseparatedissociatedcellsfromSphereCol®beads,thesamplecanbepassedthroughacellstrainer.
- SphereCol®beads/cellseparationcanalsobeperformedviadifferentialsettlinginaconicaltube.
ProductCellAssay
Todemonstratecellattachment,cellswereseededontoSphereCol®humancollagencoatedbeads.ThephotobelowshowsafluorescentimageofhumanMesenchymalStemCellsattachedtothebeads.DAPIstainednucleiappearblueandPhalloidin-Alexa-488stainingofactinfilamentsisgreen.
ProductReferences
SphereCol®References:
Park,Yonsil,etal."Hepaticdifferentiationofhumanembryonicstemcellsonmicrocarriers."Journalofbiotechnology174(2014):39-48.
Dai,Lin,etal."Inorganic–organicnanocompositeassemblyusingcollagenasatemplateandsodiumtripolyphosphateasabiomimeticanalogofmatrixphosphoprotein."Crystalgrowth&design11.8(2011):3504-3511.
Rafiq,QasimA.,etal."Systematicmicrocarrierscreeningandagitatedcultureconditionsimproveshumanmesenchymalstemcellyieldinbioreactors."Biotechnologyjournal11.4(2016):473-486.
Lin,YoushanMelissa,etal."Criticalattributesofhumanearlymesenchymalstromalcell-ladenmicrocarrierconstructsforimprovedchondrogenicdifferentiation."Stemcellresearch&therapy8.1(2017):93.
Yoon,Junghyo,etal."FabricationoftypeIcollagenmicrocarrierusingamicrofluidic3DT-junctiondeviceanditsapplicationforthequantitativeanalysisofcell–ECMinteractions."Biofabrication8.3(2016):035014.
Rafiq,QasimA."TowardascalableandconsistentmanufacturingprocessfortheproductionofhumanMSCs."CellandGeneTherapyInsights2.1(2016):127-140.
Wang,Zhenxing,etal."Developmentofdemineralizedbonematrix-basedimplantableandbiomimeticmicrocarrierforstemcellexpansionandsingle-steptissue-engineeredbonegraftconstruction."JournalofMaterialsChemistryB5.1(2017):62-73.
Suess,P.M.,Chinea,L.E.,Pilling,D.&Gomer,R.H.ExtracellularPolyphosphatePromotesMacrophageandFibrocyteDifferentiation,InhibitsLeukocyteProliferation,andActsasaChemotacticAgentforNeutrophils.TheJournalofImmunology(2019).doi:10.4049/jimmunol.1801559
Tavassoli,H.etal.Large-scaleproductionofstemcellsutilizingmicrocarriers:ABiomaterialsengineeringperspectivefromacademicresearchtocommercializedproducts.Biomaterials181,333–346(2018).
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ThisproductisforR&Duseonlyandisnotintendedforhumanorotheruses.PleaseconsulttheMaterialSafetyDataSheetforinformationregardinghazardsandsafehandlingpractices.
